Supramolecular Interaction of Fullerenes with a Curved π‐Surface of a Monomeric Quadruply Ring‐Fused Porphyrin

Molecular binding of fullerenes, C₆₀ and C₇₀, with the Zn^II complex of a monomeric ring‐fused porphyrin derivative ( 2 ‐py) as a host molecule, which has a concave π‐conjugated surface, has been confirmed spectroscopically. The structures of associated complexes composed of fullerenes and 2 ‐py were explicitly established by X‐ray diffraction analysis. The fullerenes in the 2:1 complexes, which consist of two 2 ‐py molecules and one fullerene molecule, are fully covered by the concave surfaces of the two 2 ‐py molecules in the crystal structure. In contrast, in the crystal structure of the 1:1 complex consisting of one 2 ‐py molecule and one C₆₀ molecule, the C₆₀ molecule formed a π–π stacked pair with a C₆₀ molecule in the neighboring complex using a partial surface, which was uncovered by the 2 ‐py molecule. Additionally, the molecular size of fullerene adopted significantly affects the ¹H NMR spectral changes and the redox properties of 2 ‐py upon the molecular binding.     

Cucurbit[7]uril: A High‐Affinity Host for Encapsulation of Amino Saccharides and Supramolecular Stabilization of Their α‐Anomers in Water

Cucurbit[7]uril (CB[7]), an uncharged and water‐soluble macrocyclic host, binds protonated amino saccharides (D ‐glucosamine, D ‐galactosamine, D ‐mannosamine and 6‐amino‐6‐deoxy‐D ‐glucose) with excellent affinity (K_a=10³ to 10⁴ M ^?1). The host–guest complexation was confirmed by NMR spectroscopy, isothermal titration calorimetry (ITC), and MALDI‐TOF mass spectral analyses. NMR analyses revealed that the amino saccharides, except D ‐mannosamine, are bound as α‐anomers within the CB[7] cavity. ITC analyses reveal that CB[7] has excellent affinity for binding amino saccharides in water. The maximum affinity was observed for D ‐galactosamine hydrochloride (K_a=1.6×10⁴ M ^?1). Such a strong affinity for any saccharide in water using a synthetic receptor is unprecedented, as is the supramolecular stabilization of an α‐anomer by the host.     

Conformational analysis of the disaccharide methyl α‐d‐mannopyranosyl‐(1→3)‐2‐O‐acetyl‐β‐d‐mannopyranoside monohydrate

The crystal structure of methyl α‐d ‐mannopyranosyl‐(1→3)‐2‐O‐acetyl‐β‐d ‐mannopyranoside monohydrate, C₁₅H₂₆O₁₂·H₂O, ( II ), has been determined and the structural parameters for its constituent α‐d ‐mannopyranosyl residue compared with those for methyl α‐d ‐mannopyranoside. Mono‐O‐acetylation appears to promote the crystallization of ( II ), inferred from the difficulty in crystallizing methyl α‐d ‐mannopyranosyl‐(1→3)‐β‐d ‐mannopyranoside despite repeated attempts. The conformational properties of the O‐acetyl side chain in ( II ) are similar to those observed in recent studies of peracetylated mannose‐containing oligosaccharides, having a preferred geometry in which the C2—H2 bond eclipses the C=O bond of the acetyl group. The C2—O2 bond in ( II ) elongates by ～0.02 Å upon O‐acetylation. The phi (?) and psi (ψ) torsion angles that dictate the conformation of the internal O‐glycosidic linkage in ( II ) are similar to those determined recently in aqueous solution by NMR spectroscopy for unacetylated ( II ) using the statistical program MA′AT, with a greater disparity found for ψ (Δ = ～16°) than for ? (Δ = ～6°).     

Synthesis of a Fusion‐Isomeric Cellobionoimidazole and Its Evaluation against the syn‐Protonating Glycosidase Cel7A

The fusion‐isomeric cellobinoimidazole 2 , a potential inhibitor of the syn‐protonating β‐glycosidase Cel7A, was synthesised by Koenigs–Knorr glycosylation of the α‐D ‐arabinopyranoside 32 , followed by selective hydrolysis. Glycosylation of 32 with acetobromoglucose 6 proceeded with poor diastereoselectivity, giving the desired 1,3‐linked β‐d‐ disaccharide 35 as minor product, besides the major 1,3‐linked α‐d‐ disaccharide 36 . Hg²⁺‐Promoted glycosylation of 32 led predominantly to the 1,2‐ortho ester 33 . Sequential removal of the silyl, acetyl, and allyl groups of 35 led to a 45 : 55 equilibrium mixture 2 and the manno‐configured isomer 39 . Similarly, deprotection of 36 gave a mixture of the maltonoimidazole 42 and the manno‐configured isomer 43 . According to a known protocol, the glycosyl acceptor 32 was synthesised in eleven steps and an overall yield of 8–13% from D ‐lyxose. The silylated arabinopyranosyl moiety of the α‐d‐ glucosides 13 – 19, 33, 34 , and 36 adopts a ⁴C₁ conformation, while the arabinopyranosyl moiety of the β‐d‐ glucosides 17 and 35 exists as a 1 : 3 mixture of ⁴C₁ and ¹C₄ conformers, as a result of the combined preferred axial orientation of bulky vicinal substituents and the anomeric effect. MM3* Modelling evidences a preferred ⁴C₁ conformation of 35 and 36 , and stronger steric interactions between the pyranosyl moieties of 35 . The equilibrium mixture 2 / 39 proved a poor inhibitor of Cel7A with an IC₅₀ value of ca. 4 mM .     

Peracetylated α‐d‐glucopyranosyl fluoride and peracetylated α‐maltosyl fluoride

The X‐ray analyses of 2,3,4,6‐tetra‐O‐acetyl‐α‐d ‐glucopyranosyl fluoride, C₁₄H₁₉FO₉, (I), and the corresponding maltose derivative 2,3,4,6‐tetra‐O‐acetyl‐α‐d ‐glucopyranosyl‐(1→4)‐2,3,6‐tri‐O‐acetyl‐α‐d ‐glucopyranosyl fluoride, C₂₆H₃₅FO₁₇, (II), are reported. These add to the series of published α‐glycosyl halide structures; those of the peracetylated α‐glucosyl chloride [James & Hall (1969). Acta Cryst. A 25 , S196] and bromide [Takai, Watanabe, Hayashi & Watanabe (1976). Bull. Fac. Eng. Hokkaido Univ. 79 , 101–109] have been reported already. In our structures, which have been determined at 140 K, the glycopyranosyl ring appears in a regular ⁴C₁ chair conformation with all the substituents, except for the anomeric fluoride (which adopts an axial orientation), in equatorial positions. The observed bond lengths are consistent with a strong anomeric effect, viz. the C1—O5 (carbohydrate numbering) bond lengths are 1.381 (2) and 1.381 (3) Å in (I) and (II), respectively, both significantly shorter than the C5—O5 bond lengths, viz. 1.448 (2) Å in (I) and 1.444 (3) Å in (II).     

Pendant structure governed anion sensing property for sulfonamide‐functionalized poly(phenylacetylene)s bearing various α‐amino acids

The colorimetric detection of anionic species has been studied for α‐amino acid‐conjugated poly(phenylacetylene)s, which were prepared by the polymerization of the ethyl esters of N‐(4‐ethynylphenylsulfonyl)‐L ‐alanine, L ‐isoleucine, L ‐valine, L ‐phenylalanine, L ‐aspartic acid, and L ‐glutamic acid using Rh⁺(2,5‐norbornadiene)[(η⁶‐C₆H₅)B^?(C₆H₅)₃] as the catalyst in CHCl₃. The one‐handed helical conformations of all the sulfonamide‐functionalized polymers were characterized by Cotton effects in the circular dichroism spectra. The addition of anions with a relatively high basicity, such as tetra‐n‐butylammonium acetate and fluoride, induced drastic changes in both the optical and chiroptical properties. On the other hand, anions with a relatively low basicity, such as tetra‐n‐butylammonium nitrate, azide, and bromide, had essentially no effects on the helical conformation of all the sulfonamide‐functionalized polymers. The anion signaling property of the sulfonamide‐functionalized polymers possessing α‐amino acid moieties was significantly affected by the installed residual amino acid structures. © 2010 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem 48: 1683–1689, 2010     

Syntheses and Spectroscopic Study of Some New N‐4‐Fluorobenzoyl Phosphoric Triamides; Crystal Structures of 4‐F‐C6H4C(O)N(H)P(O)R2, R = NH‐C(CH3)3, NH‐CH2C6H5, N(CH3)(CH2C6H5)

Some new N‐4‐Fluorobenzoyl phosphoric triamides with formula 4‐F‐C₆H₄C(O)N(H)P(O)X₂, X = NH‐C(CH₃)₃ ( 1 ), NH‐CH₂‐CH=CH₂ ( 2 ), NH‐CH₂C₆H₅ ( 3 ), N(CH₃)(C₆H₅) ( 4 ), NH‐CH(CH₃)(C₆H₅) ( 5 ) were synthesized and characterized by ¹H, ¹³C, ³¹P NMR, IR and Mass spectroscopy and elemental analysis. The structures of compounds 1 , 3 and 4 were investigated by X‐ray crystallography. The P=O and C=O bonds in these compounds are anti. Compounds 1 and 3 form one dimensional polymeric chain produced by intra‐ and intermolecular ‐P=O···H‐N‐ hydrogen bonds. Compound 4 forms only a centrosymmetric dimer in the crystalline lattice via two equal ‐P=O···H‐N‐ hydrogen bonds. ¹H and ¹³C NMR spectra show two series of signals for the two amine groups in compound 1 . This is also observed for the two α‐methylbenzylamine groups in 5 due to the presence of chiral carbon atom in molecule. ¹³C NMR spectrum of compound 4 shows that ²J(P,C_aliphatic) coupling constant for CH₂ group is greater than for CH₃ in agreement with our previous study. Mass spectra of compounds 1 ‐ 3 (containing 4‐F‐C₆H₄C(O)N(H)P(O) moiety) indicate the fragments of amidophosphoric acid and 4‐F‐C₆H₄CN⁺ that formed in a pseudo McLafferty rearrangement pathway. Also, the fragments of aliphatic amines have high intensity in mass spectra.     

Methyl 4‐O‐β‐d‐galactopyranosyl α‐d‐mannopyranoside methanol 0.375‐solvate

Methyl β‐d ‐galactopyranosyl‐(1→4)‐α‐d ‐mannopyranoside methanol 0.375‐solvate, C₁₃H₂₄O₁₁·0.375CH₃OH, (I), was crystallized from a methanol–ethanol solvent system in a glycosidic linkage conformation, with ϕ′ (O5_Gal—C1_Gal—O1_Gal—C4_Man) = −68.2 (3)° and ψ′ (C1_Gal—O1_Gal—C4_Man—C5_Man) = −123.9 (2)°, where the ring is defined by atoms O5/C1–C5 (monosaccharide numbering); C1 denotes the anomeric C atom and C6 the exocyclic hydroxymethyl C atom in the βGalp and αManp residues, respectively. The linkage conformation in (I) differs from that in crystalline methyl α‐lactoside [methyl β‐d ‐galactopyranosyl‐(1→4)‐α‐d ‐glucopyranoside], (II) [Pan, Noll & Serianni (2005). Acta Cryst. C 61 , o674–o677], where ϕ′ is −93.6° and ψ′ is −144.8°. An intermolecular hydrogen bond exists between O3_Man and O5_Gal in (I), similar to that between O3_Glc and O5_Gal in (II). The structures of (I) and (II) are also compared with those of their constituent residues, viz. methyl α‐d ‐mannopyranoside, methyl α‐d ‐glucopyranoside and methyl β‐d ‐galactopyranoside, revealing significant differences in the Cremer–Pople puckering parameters, exocyclic hydroxymethyl group conformations and intermolecular hydrogen‐bonding patterns.     

Structural properties of D‐mannopyranosyl rings containing O‐acetyl side‐chains

The crystal structures of 1,2,3,4,6‐penta‐O‐acetyl‐α‐d ‐mannopyranose, C₁₆H₂₂O₁₁, and 2,3,4,6‐tetra‐O‐acetyl‐α‐d ‐mannopyranosyl‐(1→2)‐3,4,6‐tri‐O‐acetyl‐α‐d ‐mannopyranosyl‐(1→3)‐1,2,4,6‐tetra‐O‐acetyl‐α‐d ‐mannopyranose, C₄₀H₅₄O₂₇, were determined and compared to those of methyl 2,3,4,6‐tetra‐O‐acetyl‐α‐d ‐mannopyranoside, methyl α‐d ‐mannopyranoside and methyl α‐d ‐mannopyranosyl‐(1→2)‐α‐d ‐mannopyranoside to evaluate the effects of O‐acetylation on bond lengths, bond angles and torsion angles. In general, O‐acetylation exerts little effect on the exo‐ and endocyclic C—C and endocyclic C—O bond lengths, but the exocyclic C—O bonds involved in O‐acetylation are lengthened by ～0.02 Å. The conformation of the O‐acetyl side‐chains is highly conserved, with the carbonyl O atom either eclipsing the H atom attached to a 2°‐alcoholic C atom or bisecting the H—C—H bond angle of a 1°‐alcoholic C atom. Of the two C—O bonds that determine O‐acetyl side‐chain conformation, that involving the alcoholic C atom exhibits greater rotational variability than that involving the carbonyl C atom. These findings are in good agreement with recent solution NMR studies of O‐acetyl side‐chain conformations in saccharides. Experimental evidence was also obtained to confirm density functional theory (DFT) predictions of C—O and O—H bond‐length behavior in a C—O—H fragment involved in hydrogen bonding.     

Cyclic lipoundecapeptide tensin from Pseudomonas fluorescens strain 96.578

The crystal structure of the non‐ribosomal lipoundecapeptide tensin from Pseudomonas fluorescens has been solved as an ethyl acetate/bis‐water solvate (tensin ethyl acetate dihydrate, C₆₇H₁₁₅N₁₂O₂₀·C₄H₈O₂·2H₂O) to a resolution of 0.8 Å. The primary structure of tensin is β‐hydroxydecanoyl‐d ‐Leu‐d ‐Asp‐d ‐allo‐Thr‐d ‐Leu‐d ‐Leu‐d ‐Ser‐l ‐Leu‐d ‐Gln‐l ‐Leu‐l ‐Ile‐l ‐Glu. The peptide is a lactone linking the Thr3 O_γ atom to the C‐terminal C atom. The stereochemistry of the β‐hydroxy acid has been shown to be S. The peptide shows structural resemblance to the non‐ribosomal cyclic lipopeptide fengycin from Bacillus subtilis. The structure of tensin is essentially helical (3₁₀‐helix), with the cyclic peptide wrapping around a hydrogen‐bonded water molecule. The lipopeptide is amphipathic in good agreement with its function as a biosurfactant.     

A one‐dimensional double‐chain coordination polymer: [Mn(C12H13NO6S)(C10H8N2)]n

In the title compound, poly­[[(2,2′‐bi­pyridine‐κ²N,N′)­manganese(II)]‐μ₃‐N‐tosyl‐l ‐glutamato‐κ⁴O,O′:O′′:O′′′], [Mn(tsgluo)(bipy)]_n, where tsgluo is N‐tosyl‐l ‐glutamate (C₁₂H₁₃NO₆S) and bipy is 2,2′‐bi­pyridine (C₁₀H₈N₂), the Mn atoms are octahedrally coordinated by two N atoms of one bipy ligand and by four O atoms of three tsgluo²⁻ anions. The γ‐carboxyl group coordinates to the Mn^II atom in a chelating mode, while the α‐carboxyl group coordinates in a bidentate–bridging mode. The complex displays a one‐dimensional double‐chain structure.     

A pipecolic acid (Pip)‐containing dipeptide,Boc‐d‐Ala‐l‐Pip‐NHiPr

The title dipeptide, 1‐(tert‐butoxy­carbonyl‐d ‐alanyl)‐N‐iso­propyl‐l ‐pipecol­amide or Boc‐d ‐Ala‐l ‐Pip‐NHⁱPr (H‐Pip‐OH is pipecolic acid or piperidine‐2‐carboxylic acid), C₁₇H₃₁N₃­O₄, with a d –l heterochiral sequence, adopts a type II′β‐­turn conformation, with all‐trans amide functions, where the C‐terminal amide NH group interacts with the Boc carbonyl O atom to form a classical i+3 i intramolecular hydrogen bond. The C^α substituent takes an axial position [H^α (Pip) equatorial] and the trans pipecolamide function is nearly planar.     

Molecular aggregation in selected crystalline 1:1 complexes of hydrophobic d‐ and l‐amino acids. IV. The l‐phenylalanine series

The amino acid l ‐phenylalanine has been cocrystallized with d ‐2‐aminobutyric acid, C₉H₁₁NO₂·C₄H₉NO₂, d ‐norvaline, C₉H₁₁NO₂·C₅H₁₁NO₂, and d ‐methionine, C₉H₁₁NO₂·C₅H₁₁NO₂S, with linear side chains, as well as with d ‐leucine, C₉H₁₁NO₂·C₆H₁₃NO₂, d ‐isoleucine, C₉H₁₁NO₂·C₆H₁₃NO₂, and d ‐allo‐isoleucine, C₉H₁₁NO₂·C₆H₁₃NO₂, with branched side chains. The structures of these 1:1 complexes fall into two classes based on the observed hydrogen‐bonding pattern. From a comparison with other l :d complexes involving hydrophobic amino acids and regular racemates, it is shown that the structure‐directing properties of phenylalanine closely parallel those of valine and isoleucine but not those of leucine, which shares side‐chain branching at C^γ with phenylalanine and is normally considered to be the most closely related non‐aromatic amino acid.     

The structure of a valinomycin–hexaaquamagnesium trifluoromethanesulfonate compound

Valinomycin is a naturally occurring cyclic dodecadepsipeptide with the formula cyclo‐[d ‐HiVA→l ‐Val →l ‐LA→l ‐Val]₃ (d ‐HiVA is d ‐α‐hydroxyisovaleic acid, Val is valine and LA is lactic acid), which binds a K⁺ ion with high selectively. In the past, several cation‐binding modes have been revealed by X‐ray crystallography. In the K⁺, Rb⁺ and Cs⁺ complexes, the ester O atoms coordinate the cation with a trigonal antiprismatic geometry, while the six amide groups form intramolecular hydrogen bonds and the network that is formed has a bracelet‐like conformation (Type 1 binding). Type 2 binding is seen with the Na⁺ cation, in which the valinomycin molecule retains the bracelet conformation but the cations are coordinated by only three ester carbonyl groups and are not centrally located. In addition, a picrate counter‐ion and a water molecule is found at the center of the valinomycin bracelet. Type 3 binding is observed with divalent Ba²⁺, in which two cations are incorporated, bridged by two anions, and coordinated by amide carbonyl groups, and there are no intramolecular amide hydrogen bonds. In this paper, we present a new Type 4 cation‐binding mode, observed in valinomycin hexaaquamagnesium bis(trifluoromethanesulfonate) trihydrate, C₅₄H₉₀N₆O₁₈·[Mg(H₂O)₆](CF₃SO₃)₂·3H₂O, in which the valinomycin molecule incorporates a whole hexaaquamagnesium ion, [Mg(H₂O)₆]²⁺, via hydrogen bonding between the amide carbonyl groups and the hydrate water H atoms. In this complex, valinomycin retains the threefold symmetry observed in Type 1 binding, but the amide hydrogen‐bond network is lost; the hexaaquamagnesium cation is hydrogen bonded by six amide carbonyl groups. ¹H NMR titration data is consistent with the 1:1 binding stoichiometry in acetonitrile solution. This new cation‐binding mode of binding a whole hexaaquamagnesium ion by a cyclic polypeptide is likely to have important implications for the study of metal binding with biological models under physiological conditions.     

Brucine salts of l‐α‐hydr­oxy acids: brucinium hydrogen (S)‐malate penta­hydrate and anhydrous brucinium hydrogen (2R,3R)‐tartrate at 130 K

The structures of two brucinium (2,3‐dimeth­oxy‐10‐oxostrychnidinium) salts of the α‐hydr­oxy acids l ‐malic acid and l ‐tartaric acid, namely brucinium hydrogen (S)‐malate penta­hydrate, C₂₃H₂₇N₂O₄⁺·C₄H₅O₅⁻·5H₂O, (I), and anhydrous brucinium hydrogen (2R,3R)‐tartrate, C₂₃H₂₇N₂O₄⁺·C₄H₅O₆⁻,(II), have been determined at 130 K. Compound (I) has two brucinium cations, two hydrogen malate anions and ten water mol­ecules of solvation in the asymmetric unit, and forms an extensively hydrogen‐bonded three‐dimensional framework structure. In compound (II), the brucinium cations form the common undulating brucine sheet substructures, which accommodate parallel chains of head‐to‐tail hydrogen‐bonded tartrate anion species in the inter­stitial cavities.     

Enantiomeric and Diastereomeric Self‐Assembled Multivalent Nanostructures: Understanding the Effects of Chirality on Binding to Polyanionic Heparin and DNA

A family of four self‐assembling lipopeptides containing Ala‐Lys peptides attached to a C₁₆ aliphatic chain were synthesised. These compounds form two enantiomeric pairs that bear a diastereomeric relationship to one another (C₁₆‐l ‐Ala‐l ‐Lys/C₁₆‐d ‐Ala‐d ‐Lys) and (C₁₆‐d ‐Ala‐l ‐Lys/C₁₆‐l ‐Ala‐d ‐Lys). These diastereomeric pairs have very different critical micelle concentrations (CMCs). The self‐assembled multivalent (SAMul) systems bind biological polyanions as a result of the cationic lysine groups on their surfaces. For heparin binding, there was no significant enantioselectivity, but there was a binding preference for the diastereomeric assemblies with lower CMCs. Conversely, for DNA binding, there was significant enantioselectivity for systems displaying d ‐lysine ligands, with a further slight preference for attachment to l ‐alanine, with the CMC being irrelevant.     

Synthesis reactivity and electrochemical properties of substituted cyclopentadienyl cobalt (III) complexes

Cyclopentadienyl cobalt complexes (η⁵‐C₅H₄R) CoLI₂ [L = CO,R=‐COOCH₂CH=CH₂ (3); L=PPh₃, R=‐COOCH₂‐CH=CH₂ (6); L=P(p‐C₆H₄O₃)₃, R = ‐COOC(CH₃) = CH₂ (7), ‐COOCH₂C₆H₅ (8), ‐COOCH₂CH = CH₂ (9)] were prepared and characterized by elemental analyses, ¹H NMR, ER and UV‐vis spectra. The reaction of complexes (η⁵‐C₅H₄R)CoLI₂ [L= CO, R= ‐COOC(CH₃) = CH₂ (1), ‐COOCH₂C₆H₅(2); L=PPh₃, R=‐COOC (CH₃) = CH₂ (4), ‐COOCH₂C₆H₅ (5)] with Na‐Hg resulted in the formation of their corresponding substituted cobaltocene (η⁵‐C₅H₄R)₂ Co[R=‐COOC(CH₃) = CH₂ (10), ‐COOCH₂C₆H₅ (11)]. The electrochemical properties of these complexes 1–11 were studied by cyclic voltammetry. It was found that as the ligand (L) of the cobalt (III) complexes changing from CO to PPh₃ and P(p‐tolyl)₃, their oxidation potentials increased gradually. The cyclic voltammetry of α,α′‐substituted cobaltocene showed reversible oxidation of one electron process.     

Synthesis of glycosyl esters from phosphoroates derivatives of 2‐bromosugars

This work presents the synthesis of glycosyl esters of 2‐bromo‐2‐deoxy‐D ‐hexopyranose, having the α‐D ‐manno ( 10a–cα ), β‐D ‐gluco ( 11a–dβ ) and α‐D ‐gluco ( 11a,bα ) configuration, by a stereoselective reaction between phosphoroates 3–8 and carboxylic acids 9a–d. Derivatives of 10a–c and 11a–d are formed in an overall quantitative yield, in an aprotic solvent in the presence of silver salts as a leaving group activator. The phosphoroselenoate of 3 was obtained by the condensation reaction of the triethylammonium salt of phosphoroseleno acid 2 with α‐1,2‐D ‐manno‐pyranosyl dibromide 1 with high stereoselectivity. The structures of the compounds 3,10a–c and 11a–d were established by ¹H and ¹³C NMR spectra and by elemental analyses. © 2000 John Wiley & Sons, Inc. Heteroatom Chem 11:292–298, 2000     

Nano‐Saturn: Experimental Evidence of Complex Formation of an Anthracene Cyclic Ring with C60

An anthracene cyclic hexamer was synthesized by the coupling reaction as a macrocyclic hydrocarbon host. This disk‐shaped host included a C₆₀ guest in 1:1 ratio to form a Saturn‐type supramolecular complex in solution and in crystals. X‐ray analysis unambiguously revealed that the guest molecule was accommodated in the middle of the host cavity with several CH???π contacts. The association constant K_a determined by NMR titration measurements was 2.3×10³ L mol^?1 at 298 K in toluene. The structural features and the role of CH???π interactions are discussed with the aid of DFT calculations.